Method for antigen-specific stimulation of T lymphocytes with synthetic peptide libraries

ABSTRACT

The invention relates to a method for the antigen-specific stimulation of T-lymphocytes with a synthetic peptide library, by preparing a plurality of peptides, each of said peptides comprising a fragment less than the whole of the total amino acid sequence of the antigen, each of said peptides being a minimum of 9 amino acid residues (AAs) in length, and the amino acid sequence of each peptide overlapping with the amino acid sequence of at least one other of said peptides; combining a plurality of the peptides from a) into a peptide library, said peptide library comprises a plurality of the peptides selected such that their collective overlapping amino acid sequences span the total amino acid sequence of the antigen; and incubating a suspension comprising CD8+ T lymphocytes, CD4+ T lymphocytes or a mixture of CD8+ and CD4+ with said peptide library in a single culture run.

This application is a 371 of PCT/EP01/01773, filed Feb. 17, 2001.

The invention relates to a method for antigen-specific stimulation of T lymphocytes with synthetic peptide libraries, comprising the following steps:

-   -   (a) subdividing the total amino acid sequence of the antigen         into protein fragments with partial amino acid sequences;     -   (b) synthesizing a peptide library containing these protein         fragments;     -   (c) incubating a suspension containing CD8+ and/or CD4+ T         lymphocytes with all the protein fragments of the peptide         library in a single culture run.

The method can be employed for both the immunostimulation of T lymphocytes of mammals, especially humans, and for diagnostics in order to establish whether a mammal, especially a human, has previously responded to a specific protein with its immune system, and if so, how strong such response is.

BACKGROUND OF THE INVENTION

The immune response of CD8+ T lymphocytes to protein antigens can be detected only with a great expenditure using known methods. It depends on the presentation of the epitopes derived from these antigens on MHC class I molecules on cells and can be measured through measuring a cytotoxic response induced by exposure. This experimental set-up is usual and takes one to several weeks in which the CD8+ T lymphocytes must be stimulated with the antigen in a suitable cell culture and are then incubated in a cytotoxicity test with suitable target cells which have been loaded with peptides from this antigen or transfected with the antigen or parts thereof. The induction of a response of the CD8+ T lymphocytes is measured from the degree of destruction of target cells, which requires suitable controls and includes a great experimental and time expenditure.

The detection of the immune response of CD4+ T lymphocytes to protein antigens is somewhat less complicated. The response of CD4+ T lymphocytes to protein antigens depends on the presentation of the epitopes derived from these antigens on MHC class II molecules on cells and can be measured through the proliferation of such cells in the presence of the antigen or upon exposure to this antigen, e.g., through the incorporation of tritiated thymidine. This experimental set-up is usual and takes several days up to a week or longer. The presence of a CD4+ T lymphocyte response to protein antigens can further be measured in a known method in which a suspension containing CD4+ T lymphocytes is incubated with the corresponding protein followed by detecting the CD4+ T lymphocyte induction through the presence of intracellular cytokines by flow cytometry.

The presence of a CD8+ T lymphocyte or CD4+ T lymphocyte response to individual epitopes can further be measured in a known method in which a suspension containing CD8+ and/or CD4+ T lymphocytes is incubated with peptides from this protein followed by detecting the CD8+ or CD4+ T lymphocyte induction through the presence of intracellular cytokines by flow cytometry, making use of the fact that peptides can be charged directly from outside onto the MHC class I or MHC class II molecules on cells, circumventing intracellular processing. In this method, it can be achieved by a suitable grouping of peptides that stimulating peptides can be identified and thus epitopes can be determined. The grouping used in this way distributes all possible epitopes to several, and mostly a large number of, runs so that it can be established whether individual peptides from this protein can induce a T lymphocyte response and it can be established which of the peptides occurring in the individual groups have led to such stimulation (this is described in F. Kern et al., Journal of Virology, October 1999, p. 8179-8184, and in WO 99/36568).

However, this grouping allows neither to determine systematically in a single measurement with a corresponding control whether a T lymphocyte response against the protein is present at all, nor to tell how strong the response (the proportion of the reactive lymphocytes in percent of the total CD8+ or CD4+ T lymphocytes) to this protein is all in all. To do this, the usual grouping in this method for the identification of epitopes would require several stimulation and measuring runs, depending on the number of peptides used. The application described in the literature aims at the precise identification of epitopes and therefore uses groups of peptides whose size is chosen in such a way that as few as possible individual peptides must be tested to establish the stimulating activity of a peptide group. However, the smaller the group size is chosen, the more groups have to be tested. Therefore, as the most favorable variant, a number of groups is chosen in this method which is twice the square root of the next square number exceeding the number of the peptides (unless the number of peptides is itself a square number).

This may be exemplified by the pp65 protein of the human cytomegalovirus. 138 peptides were synthesized which cover the amino acid sequence of the whole protein (561 amino acids) to the full length thereof, neighboring peptides overlapping by 9 amino acids each. 138 is not a square number. The next higher square number from 138 is 144 (12×12). Thus, the peptides were distributed to 2×12, i.e. 24, groups in such a way that each peptide occurs in exactly two different groups. By combining the groups with positive results (stimulation), the stimulating peptide can be concluded directly (when only two groups show a positive result), or it can be narrowed down to a small number of candidate peptides which can be retested individually, if more then two groups of peptides have resulted in positive stimulation results. The principle of this grouping has been described in some detail by F. Kern et al., Journal of Virology, October 1999, p. 8179-8184. A possibility for telling by one single run with a corresponding negative control whether a protein has a stimulating effect on CD8+ T lymphocytes, i.e., whether the amino acid sequence of this protein contains epitopes which are recognized by CD8+ T lymphocytes, has not been described to date.

DESCRIPTION OF THE INVENTION

The object of the invention is to provide a possibility for how to employ protein antigens of known sequence for the immunostimulation of CD8+ and CD4+ T lymphocytes, wherein cellular antigen processing is not necessary and individual antigenic determinants (epitopes) need not be identified. It has now been found that a sufficient immunostimulation can be achieved by incubation with T lymphocytes of a special peptide library of individual fragments of the antigen with some overlapping of the fragments. The stimulation can be detected by flow cytometry. Thus, it can be established whether an organism (human or animal) has built up a T lymphocyte response against the immunizing antigen after an exposure which has occurred (also well-aimed immunization). This T lymphocyte reactivity can be examined in terms of its time course. A further object of the invention is to provide a method by which protein antigens whose amino acid sequences are known can be identified as T-lymphocyte-stimulating protein antigens within a short time and with comparably few expenditure. This further provides a possibility for examining prior to the selection of a protein for the identification of epitopes whether T-lymphocyte-stimulating antigenic determinants are at all present in this protein.

Thus, the present invention relates to

-   -   (1) a method for the antigen-specific stimulation of T         lymphocytes with synthetic peptide libraries, comprising the         following steps:         -   (a) subdividing the total amino acid sequence of the antigen             into protein fragments with partial amino acid sequences,             wherein said protein fragments have a minimum length of 9             amino acid residues (also briefly referred to as “AA” in the             following), and wherein adjacent or neighboring protein             fragments are overlapping with their partial amino acid             sequence;         -   (b) synthesizing a peptide library containing the protein             fragments defined in (a);         -   (c) incubating a suspension containing CD8+ and/or CD4+ T             lymphocytes with all the protein fragments of the peptide             library obtained in (b) in a single culture run;     -   (2) in a preferred embodiment of method (1), it is adapted for         in-vivo and in-vitro immunostimulation of T lymphocytes of         mammals, especially humans;     -   (3) stimulated T lymphocytes obtainable by the method as defined         above under (2);     -   (4) use of a peptide library as defined above under (1) for the         preparation of a medicament for in-vivo immunostimulation of T         lymphocytes of mammals; and     -   (5) a composition for in-vitro and in-vivo immunostimulation of         T lymphocytes of mammals, comprising one or more peptide         libraries as defined above under (1).

DESCRIPTION OF FIGURES

FIG. 1: Peptides for whole pool HCMV IE-1 (laboratory strain AD169). The sequence of the starting protein, VIE1-HCMVA 55 kDa immediate-early protein 1 (IE1), human cytomegalovirus (strain AD169), is known from Swiss-Prot P13202 and depicted in SEQ ID NO:1.

FIG. 2: Peptides for whole pool HCMV pp65 (laboratory strain AD169). The sequence of the starting protein, PP65-HCMVA 65 kDa lower matrix phosphoprotein (pp65), human cytomegalovirus (strain AD169), is known from Swiss-Prot P06725 and depicted in SEQ ID NO:2.

FIG. 3: Detection of intracellular interferon-gamma in CD8+ T lymphocytes upon stimulation with the peptide libraries described. The marker CD69 was used as an activation marker in addition to interferon-gamma. The representation has been limited to CD3+/CD8+ events, stating the average fluorescence intensity.

DETAILED DESCRIPTION OF THE INVENTION

“Antigens” in the method according to the invention are those antigens which have a peptide basic structure (i.e., proteins, parts of proteins or polypeptides etc.). The antigen in step (a) of the above defined method is an antigen (i.e., protein, part of a protein, or polypeptide) to which a T lymphocyte stimulation is desired, or on which it is to be tested whether such a stimulation has already occurred.

“Proteins or peptides” in the present invention have a sequence of at least nine AAs as an essential feature.

A “peptide library” within the meaning of the application is a complex mixture of peptides which in their entirety cover the complete sequence of a protein antigen or partial antigen, which is in such a way that successive peptides are overlapping along this sequence.

Therefore, in the method according to embodiment (1) of the invention, it may be necessary to determine the total amino acid sequence of the antigen prior to the above mentioned step (a), especially when the amino acid sequence of the antigen is not known.

It does not matter how the sequence of the antigen has been established. Thus, for a new protein, the sequence can be analyzed for the first time, or for a known protein, it may be read from a data base. It is only important that the amino acid sequence of the protein or partial protein has been determined.

In a preferred embodiment of method (1) according to the invention, the protein fragments have a minimum length of 15 AAs and/or a maximum length of 35 AAs, preferably 25 AAs. It is further preferred that an overlap of 8 AAs, preferably 11 AAs, is present between neighboring protein fragments. In addition, the synthetic protein fragments may be extended by a maximum of 7 natural or artificial AAs and/or a protective group at either or both of their N terminus and C terminus. These extensions of natural or artificial AAs are non-overlapping sequences.

Suitable protective groups on the N terminus of the protein fragments are alkyl, aryl, alkylaryl, aralkyl, alkylcarbonyl or arylcarbonyl, having from 1 to 10 carbon atoms, an acyl group having from 1 to 7 carbon atoms, etc. Preferred protective groups for the N terminus are the naphthoyl, naphthylacetyl, naphthylpropionyl and benzoyl groups. Suitable protective groups for the C terminus of the protein fragments are alkoxy or aryloxy groups having from 1 to 10 carbon atoms or an amino group. Further protective groups are described in Houben-Weyl (1974), Georg Thieme Verlag, 4th Edition. The description of the protective groups in the above reference is included herein by reference.

Further, it is preferred that the concentration of the individual protein fragments of the peptide library is at least 1 ng/ml, preferably from about 0.1 to about 10 μg/ml in the culture run (final concentration). Particularly preferred is a concentration of about 1 μg/ml of culture broth.

In addition, it is preferred that the incubation solution (i.e., the culture broth) further contains one or more compounds having costimulatory properties, such as costimulatory antibodies (e.g. anti-CD28 or anti-CD49d) or other molecules having costimulatory properties. (e.g., stimulatory CTLA4-Ig). These compounds are preferably contained in the culture broth in final concentration of from 0.1 to 10 μg/ml.

A particularly preferred embodiment of the method (1) according to the invention for the antigen-specific stimulation of T lymphocytes with synthetic peptide libraries comprises the following steps:

-   -   (a₁) determining the total amino acid sequence of the antigen,         which is a protein or part of a protein;     -   (a₂) subdividing the total amino acid sequence in protein         fragments having partial amino acid sequences, wherein the         protein fragments have a minimum length of 9 (preferably 15)         AAs, optionally have a maximum length of 25 AAs, and wherein         adjacent or neighboring protein fragments are over-lapping with         their partial amino acid sequence, an overlap of 8 AAs,         especially an overlap of 11 AAs, being preferred;     -   (b) synthesizing a peptide library containing the protein         fragments defined in (a2), optionally extended by a maximum of 7         natural or artificial amino acids and/or a protective group at         either or both of the N terminus and C terminus;     -   (c) incubating a suspension containing CD8+ and/or CD4+ T         lymphocytes with all the protein fragments of the peptide         library in a single culture run.

Preferred is the use of the method according to the invention for identifying stimulating or non-stimulating mixtures of all protein fragments in a single culture run, wherein the following steps are added:

-   -   (d) identifying (preferably flow-cytometric identifying) of         -   (i) at least one T-cell cytokine which was induced by the             protein fragment or fragments and synthesized in the T             lymphocytes, wherein said cytokine or cytokines are             intracellular or bound to the cell membrane;         -   and/or         -   (ii) at least one activation marker which was induced by the             protein fragment or fragments and synthesized in the T             lymphocytes, wherein said activation marker or markers are             intracellular or bound to the cell membrane.

The method (1) according to the invention is also suitable for establishing whether T-lymphocyte-stimulating antigenic determinants are present in an antigen.

The method according to the invention is further suitable for diagnostics, especially to establish whether a mammal, especially a human, has previously responded to a specific protein with its immune system, and how strong such response is.

According to the preferred embodiment (2) of the invention, the method is suitable for immunostimulation of T lymphocytes of mammals, especially humans, for both in-vitro and in-vivo applications. This method may further include the expanding of the stimulated T lymphocytes.

The above mentioned embodiments of the method according to the invention may also be designed to employ several different synthetic peptide libraries (from different antigens) together in one culture run or in separated culture runs.

Suspensions containing T lymphocytes within the meaning of this application are characterized by containing cells which can present MHC-bound peptides. Thus, the presenting cells may also be T lymphocytes in addition to the antigen-presenting cells.

An advantage of the method according to the invention is the fact that the identification of at least one T-cell cytokine or activation marker is effected on the level of the individual cell. Thus, it is possible to exactly determine the phenotype of the responding cells. Cytokines and surface markers are described in some detail in Abul K. Abbas et al. (1997), Cellular and Molecular Immunology, Philadelphia, 3rd Edition, ISBN 0-7216-4024-9.

It is known that protein fragments binding to MHC class I molecules (MHC=major histocompatibility complex) usually have a length of 9 amino acids, while protein fragments binding to MHC class II molecules are somewhat longer and more variable in length.

An advantage of methods (1) and (2) according to the invention is the fact that, despite of the short incubation time, the protein fragments are taken up by the MHC molecules present on the cell surface sufficiently to enable an unambiguous identification of a T-cell stimulation after six hours, for example.

In the method according to the invention, the suspension containing T lymphocytes can be derived from whole blood, peripheral white blood cells (PWBC), splenocytes, thymocytes, bone marrow, cerebrospinal fluid, lymph node cells, etc.

In the method according to the invention, it is particularly advantageous that processing of the T lymphocytes is not required. Thus, the T lymphocytes need not be enriched, and further, the removal or destruction of other cells is not necessary. Thus, the method according to the invention can be practiced more simply in a routine manner.

Preferred is a method according to the invention for antigen-specific stimulation of T lymphocytes with synthetic peptide libraries in which the suspension containing the T lymphocytes is derived from patients to be treated, from other donors or from animals. If the suspension containing T lymphocytes is derived from a patient, the identification can be used, for example, for establishing to which protein of a virus a CD8+ or CD4+ T lymphocyte response can be induced. The peptide library employed for examining this reactivity can then be selectively employed for the stimulation of further T lymphocytes of the same or other patients. The cells thus induced and stimulated for proliferation can be expanded in vivo or ex vivo and subsequently retransfused to the patient.

The method according to the invention can also be used in veterinary medicine. It is possible to use a wide variety of animal species and also constellations of animal patients and donors as the source of the suspension containing T lymphocytes.

Advantageous is a method according to the invention for the antigen-specific stimulation of T lymphocytes with synthetic peptide libraries in which the antigens, which are proteins or partial proteins, are derived from microorganisms, macroorganisms, cells, cell cultures and/or tissues from donors or patients. Microorganisms include, for example, viruses, bacteria, fungi, protozoans, parasites. Macroorganisms include, for example, all multicellular eukaryotes. This source is just important for influencing allergies. Included are animals and plants. There may be used cells, cell cultures or even whole tissues consisting of one or more layers or cell types.

Preferred is a method according to the invention for antigen-specific stimulation of T lymphocytes with synthetic peptide libraries in which the stimulation is detected by means of a flow cytometer. What is essential is the principle that markers present in the cell or on its surface, such as cytokines or surface markers, will contact with a specific detector, for example, an antibody, the detector being loaded with a fluorescent dye. Upon excitation by laser light of this fluorescent dye on the cells focused in a liquid stream, the flow cytometer records the emitted scattered light and fluorescence signals, which enables the simultaneous or later analysis of the cells. Such techniques are described in some detail in Howard M. Shapiro (1995), Practical Flow Cytometry, New York, 3rd Edition, ISBN 0-471-30376-3. The detection of the intracellular cytokines is described in I L L. Picker et al. (1995), Blood, Vol. 86, p. 1408.

The advantage of this method according to the invention for antigen-specific stimulation of T lymphocytes with synthetic peptide libraries is that a reagent for the immunostimulation of T lymphocytes can be made available within a very short period of time and, as compared to the conventional method, with very low expenditure. It is further advantageous that individual stimulating epitopes need not to be identified.

In a single run (one tube or one well or one flask, etc.), the T lymphocytes of a donor/patient (CD8 and/or CD4) can be stimulated simultaneously with all possible antigenic determinants of the protein (or proteins when several peptide libraries are used) without needing to be specifically known. For example, the T lymphocytes of a patient who has undergone a bone marrow transplantation could be incubated with HLA-identical dendritic cells which were previously incubated with such a mixture of peptides, and thus these T lymphocytes could be stimulated with all epitopes relevant (i.e., binding) to the particular HLA type without these epitopes needing to be known or becoming known by the method. The only critical point is that they stimulate T lymphocytes and belong to the selected protein or proteins. These cells could be retransferred to the patient within the scope of an adoptive immunotherapy.

A preferred source of the T lymphocytes to be stimulated are those (human or animal) donors which have previously build up an immunological primary response to the antigen or in which such an immune response to the antigen has been induced by exposure. This may have occurred, for example, within the scope of an infection or also within the scope of an immunization. This situation also prevails in an auto-immune response.

Another advantage is that the MHC type of the donor need not be known. A further advantage is that the stimulation of both CD8+ and CD4+ T lymphocytes can be examined simultaneously and in a single run.

The stimulated T lymphocytes according to embodiment (3) of the invention are preferably obtained by in-vitro stimulation. The stimulated lymphocytes are capable of being transfused into a patient.

The medicament according to embodiment (4) of the invention may contain further immunoreactive compounds, such as the above defined compounds having co-stimulating properties, in addition to usual additives and auxiliaries. The medicament may also contain several of the above defined peptide libraries.

The composition according to embodiment (5) can be a pharmaceutical composition, i.e., for the in-vivo treatment of humans and animals, or a diagnostic composition or a so-called kit, i.e., primary for in-vitro application, wherein the peptide library is respectively adapted to the antigen to be stimulated. As to further components of the composition, the same applies as has been set forth above with respect to embodiment (4).

The present invention is further illustrated by the following non-limiting Example.

EXAMPLE

Mononuclear cells were prepared from the peripheral blood of two patients obtained by venous puncture. The patients possessed antibodies against the human cytomegalovirus (HCMV). The cells prepared by standard methods were incubated for six hours under optimized conditions with peptide libraries for the HCMV proteins 65 kD lower matrix phosphoprotein (pp65) and 55 kDa immediate-early protein 1 (IE1). This is done according to the method described in Kern et al., Eur. J. Immunol. 30: 1676-1682 (2000), which comprises the following steps:

-   -   1. Resuspension of PBMC (2.5×10⁶/ml in RPMI 1640 with 2 mM         glutamine added) after Ficoll preparation (standard protocol).     -   2. 400 μl of this suspension was mixed in an incubation vessel         (sterile tube from Falcon No. 2054, 5 ml) with 100 μl of peptide         solution (containing 10 μg of each individual peptide in RPMI         1640 with 2 mM glutamine added).     -   3. Incubation at 37° C. under an H₂O-saturated atmosphere with         5% CO₂ (standard incubator).     -   4. After 2 hours, there was added 500 μl of RPMI 1640 to which         20% fetal calf serum (v/v) and additionally glutamine (2 mM) and         10 μg of Brefeldin A (BFA, final concentration in the mix was 10         μg/ml) had been added. The final concentration of fetal calf         serum in the mix is 10% (v/v). The final concentration of each         individual peptide is 1 μg/ml. BFA serves to retain synthetic         cytokines in the cells, which is of advantage for the detection         of the intracellular cytokines. The final volume of the mix is 1         ml.     -   5. After further incubation for 4 h under the same conditions         (i.e., a total incubation time of 6 h), the incubation was         stopped by adding ice-cold PBS buffer solution.     -   6. This was followed by centrifugation (8 min, 400 g),         decantation and further processing of the samples according to a         standard protocol, including detachment from the tube wall using         2 mM EDTA/PBS solution, fixation, permeabilization and staining         with monoclonal antibodies.     -   7. Analysis on a flow cytometer (e.g., a four-color fluorescence         flow cytometer of the type FacsCalibur (Becton Dickinson)).

The sequences of IE-1 and pp65 have been deposited in the SWISS-PROT data base, European Bioinformatics Institute, under the Nos. P13202 (see also SEQ ID NO: 1) and P06725 (see also SEQ ID NO: 2). In addition, the sequences of both proteins are described in M. S. Chee, A. T. Bankier, S. Becks et al., Curr. Top. Microbiol. Immunol. 154: 125-169 (1990).

The peptide library which represents the 55 kD immediate-early protein 1 consisted of peptides of 15 amino acids length each with 9 overlaps between successive peptides (see FIG. 1), and the peptide library which represents the 65 kD lower matrix phosphoprotein consisted of peptides of 15 amino acids length each with 11 overlaps between successive peptides (see FIG. 2).

In two different individuals (columns “I)” and “II)” in FIG. 3), incubation with the peptide libraries resulted in the production of IFN-gamma in T cells, which was detected by measurement on a flow cytometer on the level of the individual cells (J. L. Picker et al. (1995), Blood, Vol. 86, p. 1408-1419), or else in no detectable stimulation. Individual I exhibited a CD8+ T lymphocyte response to IE-1, but not to pp65, whereas individual II exhibited a CD8+ T lymphocyte response to both proteins. Incubation with an irrelevant peptide did not produce this effect (control). 

1. A method for the human cytomegalovirus (HCMV) antigen-specific stimulation of T lymphocytes with a synthetic peptide library, said method comprising the following steps: a) synthesizing a peptide library of an HCMV antigen, said HCVM antigen being a whole HCMV protein of known total amino acid sequence, wherein each of the peptides of said peptide library comprises an amino acid sequence that (i) is at least 15 amino acid residues in length, (ii) is a continuous fragment less than the entirety of said total amino acid sequence, and (iii) overlaps to an extent of at least 8 amino acids with the amino acid sequence of at least one other of said peptides; and wherein the amino acid sequences of the peptides in the peptide library span the total amino acid sequence of the whole HCMV protein; b) incubating a T lymphocyte suspension comprising CD8+ T lymphocytes, CD4+ lymphocytes or a mixture of CD8+ T lymphocytes and CD4+ T lymphocytes with the peptide library in a single culture run; and c) identifying by flow-cytometry at least one result of said stimulating in b), wherein said at least one result is a release by said stimulated T lymphocytes of at least one T-cell cytokine and/or an expression by said stimulated T lymphocytes of at least one activation marker, wherein said release and expression are a result of said incubating of said T lymphocyte suspension with the peptide library in the single culture run.
 2. The method according to claim 1, wherein the peptides have a minimum length of 15 AAs and a maximum length of 35 AAs.
 3. The method according to claim 2, wherein the HCMV protein is selected from the group consisting of lower matrix phosphoprotein (pp65) and immediate-early protein 1 (1E1).
 4. The method according to claim 2, wherein the peptides are extended by a maximum of 7 AAs and/or a protective group at either or both of their N terminus and C terminus.
 5. The method according to claim 1, wherein the concentration of the individual peptides of the peptide library in the incubating suspension is at least 1 ng/ml.
 6. The method according to claim 1, wherein at least one compound that co-stimulates T lymphocytes is added to the incubating suspension.
 7. The method according to claim 1, wherein the total amino acid sequence of the protein is determined prior to step a) in the method.
 8. The method according to claim 1, which further comprises determining whether T-lymphocyte-stimulating antigenic determinants are present in the protein.
 9. The method according to claim 1, wherein the T lymphocytes are mammalian in origin.
 10. The method according to claim 9, further comprising reproducing the stimulated T lymphocytes.
 11. The method according to claim 1, wherein the peptides have a length of 25 AAs.
 12. The method according to claim 1, wherein an overlap of 11 AAs exists between overlapping peptides.
 13. The method according to claim 1, wherein the concentration of the individual peptides of the peptide library in the incubating suspension is 0.1 to 10 ug/ml. 